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发现两种组装活性[Fe]氢化酶所需的新型自由基S-腺苷甲硫氨酸蛋白。

Discovery of two novel radical S-adenosylmethionine proteins required for the assembly of an active [Fe] hydrogenase.

作者信息

Posewitz Matthew C, King Paul W, Smolinski Sharon L, Zhang Liping, Seibert Michael, Ghirardi Maria L

机构信息

National Renewable Energy Laboratory, Colorado School of Mines, Golden, CO 80401, USA.

出版信息

J Biol Chem. 2004 Jun 11;279(24):25711-20. doi: 10.1074/jbc.M403206200. Epub 2004 Apr 13.

Abstract

To identify genes necessary for the photoproduction of H(2) in Chlamydomonas reinhardtii, random insertional mutants were screened for clones unable to produce H(2). One of the identified mutants, denoted hydEF-1, is incapable of assembling an active [Fe] hydrogenase. Although the hydEF-1 mutant transcribes both hydrogenase genes and accumulates full-length hydrogenase protein, H(2) production activity is not observed. The HydEF protein contains two unique domains that are homologous to two distinct prokaryotic proteins, HydE and HydF, which are found exclusively in organisms containing [Fe] hydrogenase. In the C. reinhardtii genome, the HydEF gene is adjacent to another hydrogenase-related gene, HydG. All organisms with [Fe] hydrogenase and sequenced genomes contain homologues of HydE, HydF, and HydG, which, prior to this study, were of unknown function. Within several prokaryotic genomes HydE, HydF, and HydG are found in putative operons with [Fe] hydrogenase structural genes. Both HydE and HydG belong to the emerging radical S-adenosylmethionine (commonly designated "Radical SAM") superfamily of proteins. We demonstrate here that HydEF and HydG function in the assembly of [Fe] hydrogenase. Northern blot analysis indicates that mRNA transcripts for both the HydEF gene and the HydG gene are anaerobically induced concomitantly with the two C. reinhardtii [Fe] hydrogenase genes, HydA1 and HydA2. Complementation of the bx;1C. reinhardtii hydEF-1 mutant with genomic DNA corresponding to a functional copy of the HydEF gene restores hydrogenase activity. Moreover, co-expression of the C. reinhardtii HydEF, HydG, and HydA1 genes in Escherichia coli results in the formation of an active HydA1 enzyme. This represents the first report on the nature of the accessory genes required for the maturation of an active [Fe] hydrogenase.

摘要

为了鉴定莱茵衣藻中光产生H₂所必需的基因,对随机插入突变体进行筛选,寻找不能产生H₂的克隆。其中一个被鉴定的突变体,命名为hydEF - 1,无法组装有活性的[Fe]氢化酶。尽管hydEF - 1突变体转录了两个氢化酶基因并积累了全长氢化酶蛋白,但未观察到H₂产生活性。HydEF蛋白包含两个独特结构域,与两种不同的原核蛋白HydE和HydF同源,这两种蛋白仅在含有[Fe]氢化酶的生物体中发现。在莱茵衣藻基因组中,HydEF基因与另一个氢化酶相关基因HydG相邻。所有含有[Fe]氢化酶且基因组已测序的生物体都含有HydE、HydF和HydG的同源物,在本研究之前,它们的功能未知。在几个原核生物基因组中,HydE、HydF和HydG存在于与[Fe]氢化酶结构基因的推定操纵子中。HydE和HydG都属于新兴的自由基S - 腺苷甲硫氨酸(通常称为“自由基SAM”)超家族蛋白。我们在此证明HydEF和HydG在[Fe]氢化酶的组装中起作用。Northern印迹分析表明,HydEF基因和HydG基因的mRNA转录本在厌氧条件下与莱茵衣藻的两个[Fe]氢化酶基因HydA1和HydA2同时被诱导。用对应于HydEF基因功能拷贝的基因组DNA对莱茵衣藻hydEF - 1突变体进行互补,可恢复氢化酶活性。此外,莱茵衣藻HydEF、HydG和HydA1基因在大肠杆菌中的共表达导致形成有活性的HydA1酶。这是关于活性[Fe]氢化酶成熟所需辅助基因性质的首次报道。

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